Difference between revisions of "Team:Peking/Design"

Tuberculosis (TB), caused by Mycobacterium tuberculosis, remains one of the world's most serious public health problems. Although tuberculosis is curable and the treatment success rate is high, it is still the second most common cause of death from infectious disease. Most of the deaths occur for lack of effective identification of those in need of therapy. Case detection is currently the rate-limiting step in TB control.

The currently major TB detection methods all have their own problems. Nucleic Acid Detection (NAD) is a safer, faster, and more sensitive detection method available. However, it has short comes: the high false positive rate from non-specific amplification, and the requirement of extremely expensive clumsy instruments, which make NAD not common for TB diagnosis.

To obviate such problems, Peking iGEM developed a novel detection system that can directly read out specific sequence information inside the PCR amplified product, and convert the information into visible signal. Our PC Reporter was successfully applied to the detection of real pathogenic M.Tuberculosis H37Rv (safe isolated genomic DNA, provided by collaborator). Combined with our work in multi-marker array design and hardware development, this new advanced system can be turned out as a powerful tool in TB diagnosis, with a huge potential for applications and extensions.